Altered splicing machinery in lung carcinoids unveils NOVA1, PRPF8 and SRSF10 as novel candidates to understand tumor biology and expand biomarker discovery

Ricardo Blázquez-Encinas; Víctor García-Vioque; Teresa Caro-Cuenca; María Trinidad Moreno-Montilla; Federica Mangili; Emilia Alors-Pérez; Sebastian Ventura; Aura D Herrera-Martínez; Paula Moreno-Casado; Marco A Calzado; Ángel Salvatierra; María A Gálvez-Moreno; Lynnette Fernandez-Cuesta; Matthieu Foll; Raúl M Luque; Nicolas Alcala; Sergio Pedraza-Arevalo; Alejandro Ibáñez-Costa; Justo P Castaño

doi:10.1186/s12967-023-04754-8

Altered splicing machinery in lung carcinoids unveils NOVA1, PRPF8 and SRSF10 as novel candidates to understand tumor biology and expand biomarker discovery

J Transl Med. 2023 Dec 4;21(1):879. doi: 10.1186/s12967-023-04754-8.

Authors

Ricardo Blázquez-Encinas^#^{1

2

3}, Víctor García-Vioque^#^{1

2

3}, Teresa Caro-Cuenca^#^{1

4}, María Trinidad Moreno-Montilla^{1

2

3}, Federica Mangili^{1

2

3

5}, Emilia Alors-Pérez^{1

2

3}, Sebastian Ventura^{1

6}, Aura D Herrera-Martínez^{1

7}, Paula Moreno-Casado^{1

8}, Marco A Calzado^{1

2

3}, Ángel Salvatierra^{1

8}, María A Gálvez-Moreno^{1

7}, Lynnette Fernandez-Cuesta⁹, Matthieu Foll⁹, Raúl M Luque^{1

2

3

10}, Nicolas Alcala⁹, Sergio Pedraza-Arevalo^{1

2

3}, Alejandro Ibáñez-Costa^#^{11

12

13}, Justo P Castaño^#^{14

15

16

17}

Affiliations

¹ Maimónides Biomedical Research Institute of Córdoba (IMIBIC), Córdoba, Spain.
² Department of Cell Biology, Physiology, and Immunology, University of Córdoba, Córdoba, Spain.
³ Reina Sofia University Hospital, Córdoba, Spain.
⁴ Pathology Service, Reina Sofía University Hospital, Córdoba, Spain.
⁵ Department of Clinical Sciences and Community Health, University of Milan, Milan, Italy.
⁶ Department of Computer Sciences, University of Córdoba, Córdoba, Spain.
⁷ Endocrinology and Nutrition Service, Reina Sofia University Hospital, Córdoba, Spain.
⁸ Thoracic Surgery and Lung Transplantation Unit, Reina Sofa University Hospital, Córdoba, Spain.
⁹ Rare Cancers Genomics Team (RCG), Genomic Epidemiology Branch (GEM), International Agency for Research On Cancer (IARC/WHO), Lyon, France.
¹⁰ CIBER Fisiopatología de La Obesidad y Nutrición (CIBERobn), Córdoba, Spain.
¹¹ Maimónides Biomedical Research Institute of Córdoba (IMIBIC), Córdoba, Spain. b12ibcoa@uco.es.
¹² Department of Cell Biology, Physiology, and Immunology, University of Córdoba, Córdoba, Spain. b12ibcoa@uco.es.
¹³ Reina Sofia University Hospital, Córdoba, Spain. b12ibcoa@uco.es.
¹⁴ Maimónides Biomedical Research Institute of Córdoba (IMIBIC), Córdoba, Spain. justo@uco.es.
¹⁵ Department of Cell Biology, Physiology, and Immunology, University of Córdoba, Córdoba, Spain. justo@uco.es.
¹⁶ Reina Sofia University Hospital, Córdoba, Spain. justo@uco.es.
¹⁷ CIBER Fisiopatología de La Obesidad y Nutrición (CIBERobn), Córdoba, Spain. justo@uco.es.

^# Contributed equally.

Abstract

Background: Lung neuroendocrine neoplasms (LungNENs) comprise a heterogeneous group of tumors ranging from indolent lesions with good prognosis to highly aggressive cancers. Carcinoids are the rarest LungNENs, display low to intermediate malignancy and may be surgically managed, but show resistance to radiotherapy/chemotherapy in case of metastasis. Molecular profiling is providing new information to understand lung carcinoids, but its clinical value is still limited. Altered alternative splicing is emerging as a novel cancer hallmark unveiling a highly informative layer.

Methods: We primarily examined the status of the splicing machinery in lung carcinoids, by assessing the expression profile of the core spliceosome components and selected splicing factors in a cohort of 25 carcinoids using a microfluidic array. Results were validated in an external set of 51 samples. Dysregulation of splicing variants was further explored in silico in a separate set of 18 atypical carcinoids. Selected altered factors were tested by immunohistochemistry, their associations with clinical features were assessed and their putative functional roles were evaluated in vitro in two lung carcinoid-derived cell lines.

Results: The expression profile of the splicing machinery was profoundly dysregulated. Clustering and classification analyses highlighted five splicing factors: NOVA1, SRSF1, SRSF10, SRSF9 and PRPF8. Anatomopathological analysis showed protein differences in the presence of NOVA1, PRPF8 and SRSF10 in tumor versus non-tumor tissue. Expression levels of each of these factors were differentially related to distinct number and profiles of splicing events, and were associated to both common and disparate functional pathways. Accordingly, modulating the expression of NOVA1, PRPF8 and SRSF10 in vitro predictably influenced cell proliferation and colony formation, supporting their functional relevance and potential as actionable targets.

Conclusions: These results provide primary evidence for dysregulation of the splicing machinery in lung carcinoids and suggest a plausible functional role and therapeutic targetability of NOVA1, PRPF8 and SRSF10.

Keywords: NOVA1; Neuroendocrine neoplasms; PRPF8; Pulmonary carcinoids; RNA splicing; SRSF10.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Alternative Splicing / genetics
Biology
Biomarkers / metabolism
Carcinoid Tumor* / genetics
Carcinoid Tumor* / metabolism
Carcinoid Tumor* / pathology
Cell Cycle Proteins / metabolism
Humans
Lung / pathology
Lung Neoplasms* / pathology
Neuro-Oncological Ventral Antigen
RNA Splicing Factors / genetics
RNA-Binding Proteins / genetics
RNA-Binding Proteins / metabolism
Repressor Proteins / metabolism
Serine-Arginine Splicing Factors / genetics
Serine-Arginine Splicing Factors / metabolism

Substances

RNA-Binding Proteins
RNA Splicing Factors
Biomarkers
SRSF10 protein, human
Serine-Arginine Splicing Factors
Repressor Proteins
Cell Cycle Proteins
PRPF8 protein, human
NOVA1 protein, human
Neuro-Oncological Ventral Antigen
SRSF1 protein, human

Grants and funding

001/WHO_/World Health Organization/International